磷脂翻转酶 ATP8B1 通过建立肠道屏障功能参与了溃疡性结肠炎的发病机制。

Pim J Koelink, Valentina E Gómez-Mellado, Suzanne Duijst, Manon van Roest, Sander Meisner, Kam S Ho-Mok, Sabrina Frank, Babette S Appelman, Lysbeth Ten Bloemendaal, Georg F Vogel, Stan F J van de Graaf, Piter J Bosma, Ronald P J Oude Elferink, Manon E Wildenberg, Coen C Paulusma
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引用次数: 0

摘要

目的ATP8B1 基因突变的患者会患上进行性家族性肝内胆汁淤积症 1 型(PFIC1),这是一种严重的肝病,需要通过肝移植来挽救生命。PFIC1 患者还伴有肠道问题,包括肠道炎症和腹泻,这些问题在肝移植后会加重。在此,我们研究了 ATP8B1 的肠道功能与炎症性肠病的关系:设计:在克罗恩病(CD)或溃疡性结肠炎(UC)患者的肠道样本以及小鼠肠道炎症模型中调查 ATP8B1 的表达。用葡聚糖硫酸钠(DSS)诱导 ATP8B1 缺失的小鼠患结肠炎,并对肠道通透性进行研究。在 ATP8B1 基因敲除的 Caco2-BBE 细胞中评估上皮屏障功能。在过表达 ATP8B1-eGFP 的 Caco2-BBE 细胞中进行了共免疫沉淀实验。研究了 ATP8B1 和紧密连接蛋白在细胞以及 UC 和 PFIC1 患者活组织中的表达和定位情况:结果:ATP8B1在UC和DSS处理的小鼠中表达减少,并与紧密连接通路转录程序的减少有关。ATP8B1缺陷小鼠对DSS诱导的结肠炎极度敏感,表现为肠道屏障渗漏增加。ATP8B1 基因敲除的细胞显示屏障建立延迟,这与 Claudin-4 (CLDN4) 的水平和定位受到影响有关。CLDN4免疫组化结果显示,对照组织中的CLDN4呈紧密结合染色,而在UC和肠道PFIC1样本中,CLDN4没有正确定位:ATP8B1在肠道屏障的建立过程中起着重要作用 UC中ATP8B1水平的下调以及随后包括CLDN4在内的紧密连接蛋白定位的改变可能是UC病理生理学的一个重要机制。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
The Phospholipid Flippase ATP8B1 is Involved in the Pathogenesis of Ulcerative Colitis via Establishment of Intestinal Barrier Function.

Aims: Patients with mutations in ATP8B1 develop progressive familial intrahepatic cholestasis type 1 [PFIC1], a severe liver disease that requires life-saving liver transplantation. PFIC1 patients also present with gastrointestinal problems, including intestinal inflammation and diarrhoea, which are aggravated after liver transplantation. Here we investigate the intestinal function of ATP8B1 in relation to inflammatory bowel diseases.

Methods: ATP8B1 expression was investigated in intestinal samples of patients with Crohn's disease [CD] or ulcerative colitis [UC] as well as in murine models of intestinal inflammation. Colitis was induced in ATP8B1-deficient mice with dextran sodium sulphate [DSS] and intestinal permeability was investigated. Epithelial barrier function was assessed in ATP8B1 knockdown Caco2-BBE cells. Co-immunoprecipitation experiments were performed in Caco2-BBE cells overexpressing ATP8B1-eGFP. Expression and localization of ATP8B1 and tight junction proteins were investigated in cells and in biopsies of UC and PFIC1 patients.

Results: ATP8B1 expression was decreased in UC and DSS-treated mice, and was associated with a decreased tight junctional pathway transcriptional programme. ATP8B1-deficient mice were extremely sensitive to DSS-induced colitis, as evidenced by increased intestinal barrier leakage. ATP8B1 knockdown cells showed delayed barrier establishment that affected Claudin-4 [CLDN4] levels and localization. CLDN4 immunohistochemistry showed a tight junctional staining in control tissue, whereas in UC and intestinal PFIC1 samples, CLDN4 was not properly localized.

Conclusion: ATP8B1 is important in the establishment of the intestinal barrier. Downregulation of ATP8B1 levels in UC, and subsequent altered localization of tight junctional proteins, including CLDN4, might therefore be an important mechanism in UC pathophysiology.

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